Identification and quantitation of multiple variants in RNA virus genomes

IF 2.5 Q3 BIOCHEMICAL RESEARCH METHODS Biology Methods and Protocols Pub Date : 2024-02-03 DOI:10.1093/biomethods/bpae004
Johnny Sena, L. Karwal, Callum Bell, Nicholas Devitt, Faye Schilkey, Claire Huang, Jill Livengood, Subash Das, Hansi J Dean
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Abstract

The goal of the study was to identify and characterize RNA virus variants containing mutations spread over genomic distances greater than 5 kb. As proof of concept, high quality viral RNA of the Dengue 2 component of Takeda’s tetravalent dengue vaccine candidate (TDV-2) was used to develop an RT-PCR protocol to amplify a ∼5.3 kb cDNA segment that contains the three genetic determinants of TDV-2 attenuation. Unique molecular identifiers were incorporated into each viral cDNA molecule for PacBio library preparation to improve the quantitative precision of the observed variants at the attenuation loci. Following assay optimization, PacBio long read sequencing was validated with multiple clone-derived TDV-2 revertant variants and 4 complex revertant mixtures containing various compositions of TDV-2 and revertant viruses. : PacBio sequencing analysis correctly identified and quantified variant composition in all tested samples, demonstrating that TDV-2 revertants could be identified and characterized and supporting the use of this method in differentiation and quantification of complex variants of other RNA viruses. Long-read sequencing can identify complex RNA virus variants containing multiple mutations on a single genome molecule which is useful for in-depth genetic stability and revertant detection of live-attenuated viral vaccines, as well as research in virus evolution to reveal mechanisms of immune evasion and host cell adaption.
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识别和量化 RNA 病毒基因组中的多种变体
这项研究的目的是鉴定和描述含有基因组距离超过 5 kb 的突变的 RNA 病毒变体。 作为概念验证,利用武田公司候选四价登革热疫苗(TDV-2)中登革热 2 组份的高质量病毒 RNA 制定了 RT-PCR 方案,以扩增包含 TDV-2 衰减的三个遗传决定因素的 5.3 kb cDNA 片段。在 PacBio 文库制备过程中,每个病毒 cDNA 分子中都加入了独特的分子标识符,以提高在衰减位点观察到的变异的定量精度。在对检测方法进行优化后,PacBio 长读测序法在多个克隆衍生的 TDV-2 逆转录病毒变异体和 4 种包含不同 TDV-2 和逆录病毒成分的复杂逆录病毒混合物中进行了验证。 PacBio 测序分析正确识别并量化了所有测试样本中的变异体成分,证明 TDV-2 逆转录病毒可以被识别和定性,并支持将这种方法用于区分和量化其他 RNA 病毒的复杂变异体。 长读测序法可以鉴定单个基因组分子上包含多个变异的复杂 RNA 病毒变体,有助于深入研究减毒活疫苗的遗传稳定性和变异体检测,也有助于病毒进化研究,揭示免疫逃避和宿主细胞适应的机制。
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来源期刊
Biology Methods and Protocols
Biology Methods and Protocols Agricultural and Biological Sciences-Agricultural and Biological Sciences (all)
CiteScore
3.80
自引率
2.80%
发文量
28
审稿时长
19 weeks
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